Inhibition of four human serine proteases by substituted benzamidines

Abstract

A series of substituted benzamidines was examined for their inhibitory activity against the human serine proteases.sbd.trypsin (EC 3.4.4.4), thrombin (EC 3.4.4.13), plasmin (EC 3.4.4.14) and C1.hivin.s, a subunit of the first component of complement. The inhibition constants obtained for each enzyme were correlated with physical-chemical properties of the substituent group, using the quantitative structure-activity relationship approach. This analysis indicated that plasmin and C1.hivin.s are very similar in their interactions with substituted benzamidines. The binding of benzamidines in both enzymes was affected by electron donation from the substituent and its hydrophobicity. Thrombin-benzamidine interaction was affected only by the hydrophobicity of the substituent. Trypsin displayed a complex interaction with substituted benzamidines, and interaction was dependent on molar refractivity and molecular weight. Certain substituents deviated significantly from the interactions predicted by the analysis. These compounds, the (m- and p-amidinophenyl)pyruvic acids, when analyzed by computer modeling, suggested that direct interaction between the substituent and the enzyme surface is important in assessing the effect of substituent groups on inhibitory activity.